Global ETD Search

241	Quorum sensing in Sinorhizobium meliloti and effect of plant signals on bacterial quorum sensing Teplitski, Max I. 11 September 2002 (has links) No description available. Biology, Microbiology quorum sensing sinorhizobium meliloti rhizobium acyl homoserine lactone root mucilage plant polysaccharide glycanase stationary phase log phase proteomics swarming LuxR mass spectrometry Chlamydomonas secondary products rhizosphere
242	Inhibition du mécanisme de quorum sensing et de la formation de biofilm chez Pseudomonas aerugionsa par des composés bioactifs de Dalbergia trichocarpa (Fabaceae) / Dalbergia trichocarpa, source of natural compounds which affect quorum sensing mechanism and biofilm formation in Pseudomonas aeruginosa Rasamiravaka, Tsiry 13 June 2014 (has links) Depuis quelques décennies, les bactéries pathogènes multi-résistantes aux antibiotiques sont de plus en plus répandues dans le monde. Cette situation a suscité le besoin et l'intérêt de trouver des médicaments antibactériens avec de nouvelles cibles potentiels. La découverte des systèmes de communication de type quorum sensing (QS) régulant la virulence bactérienne représente une des cibles privilégiées pour contrôler les bactéries pathogènes autrement qu’en interférant avec leur croissance bactérienne. Dans l’écosystème naturel, un grand nombre d'organismes (Eucaryotes et Procaryotes) co-existent en synthétisant chacun de leur côté des métabolites secondaires. Les plantes, étant en permanence en contact avec des bactéries, synthétisent des métabolites secondaires capables d’inhiber l’expression des gènes de virulence chez les bactéries sans pour autant affecter ni leur croissance ni leur viabilité. Notre objectif a été de contribuer à la valorisation de la biodiversité malgache en identifiant des plantes et en y isolant les composés actifs présentant une capacité à perturber le mécanisme de QS chez P. aeruginosa PAO1, une bactérie pathogène opportuniste de l’homme, des animaux et des plantes. Dans ce but, nous avons tout d’abord réalisé un criblage d’activité anti-QS de différents flavonoïdes commerciaux. De ce criblage, la narigenine et la naringine ont été sélectionnées pour être les molécules de contrôle positif et négatif des tests d’activité anti-QS, respectivement. Par la suite, 4 espèces de Dalbergia endémique de Madagascar ont fait l’objet de criblage pour leur activité anti-QS. Ce travail a fait ressortir l’activité anti-QS très intéressante de l’écorce de D. trichocarpa à partir de laquelle nous avons isolée le composé actif nommé la coumarate de l’aldéhyde-oléanolique (OALC). Le contrôle naringénine et l’OALC ne présente aucun effets inhibiteurs sur la croissance bactérienne de P. aeruginosa PAO1 et sur l’expression du gène QS-indépendant aceA suggérant une activité d’inhibition spécifiquement liée au QS. Cependant, ces deux molécules présentent des spectres d’inhibition différente. En effet, les deux molécules diffèrent dans le sens que la naringenine n’inhibe pas l’expression du gène gacA et la motilité de type twitching contrairement à l’OALC. Ces résultats suggèrent que l’OALC et la naringénine représente des candidats potentiels pour des investigations in vivo quant à leur effet anti-QS et anti-biofilm sur des modèles infectieux d’organismes supérieurs. Par ailleurs, ils démontrent la richesse des plantes malgaches comme sources de nouvelles molécules anti-virulence ainsi que l’importance de telle investigation afin de renforcer notre arsenal thérapeutique en composé antibactérienne dans la lutte continuelle contre les bactéries pathogènes/Since few decades, multidrug resistant bacteria spread all over the world. This situation gives rise to the need and interest in finding antibacterial drugs with novel potent target. Discovery of communication system termed Quorum Sensing (QS) which regulate bacterial virulence factor represent privileged target in another way than interfering with bacterial growth. In natural ecosystem, many organisms (Eukaryotes and Prokaryotes) produce secondary metabolites. As plants are permanently in contact with bacteria, they have synthetized secondary metabolites which inhibit bacterial virulence gene expression without affecting bacterial viability. Our goal was to contribute to the valorization of Malagasy biodiversity and specifically to identify plants and isolate bioactive compound presenting ability to disrupt QS mechanism in P. aeruginosa, opportunistic pathogen bacteria in plants, animals and human. In this purpose, screening of commercial available flavonoids has been firstly carried out. From this screening, naringenin and naringin have been selected to be used as positive and negative QS inhibitor controls, respectively. Subsequently, Four Malagasy endemic Dalbergia species have been screened for their anti-QS activity. This work pointed out the interesting anti-QS activity of D. trichocarpa bark extract which led to the isolation of oleanolic aldehyde coumarate (OALC) as one major bioactive compound. At the concentration tested, naringenin and OALC did not affect P. aeruginosa PAO1 viability and didn’t reduce QS-independent aceA gene expression suggesting a specific anti-QS activity. However, these two compounds present different inhibition spectrum. Indeed, naringenin didn’t inhibit gacA gene expression and twitching motility contrarily to OALC. These results suggest that OALC and naringenin represent potent candidates for in vivo investigations in their anti-QS and anti-biofilm activity onto eukaryotes infectious model. Besides, this finding demonstrated the potent source for novel anti-virulence compounds of Malagasy flora and the importance of this kind of research to strengthen our antimicrobial therapeutic arsenal with the ongoing struggle against bacterial infection. / Doctorat en Sciences / info:eu-repo/semantics/nonPublished Biologie Sciences exactes et naturelles Quorum sensing (Microbiology) Pathogenic bacteria Virulence (Microbiology) Dalbergia Pseudomonas aeruginosa Détection du quorum Bactéries pathogènes Virulence (Microbiologie) Dalbergia Pseudomonas aeruginosa Secondary metabolites Acyl-homoserine lactone Coumarate de l’aldéhyde-oléanolique Flavonoïds Virulence/ Dalbergia tirchocarpa Quorum sensing Multidrug resistance Naringenin Naringenine Multirésistance Métabolites secondaires Acyle-homosérine lactone Flavonoïdes Dalbergia trichocarpa Virulence Oleanolic aldehyde coumarate
243	Fatores envolvidos com a mobilização de PAPI-1 / Factors involved with PAPI-1 mobilization Stefanello, Eliezer 07 May 2010 (has links) Genomas bacterianos são extremamente dinâmicos e boa parte dessa dinâmica ocorre devido a transferência horizontal e aquisição de DNA exógeno, um processo natural e fundamental para a evolução, adaptação e diversificação dos microrganismos. Ilhas genômicas são grandes regiões do cromossomo bacteriano adquiridas por transferência horizontal e estão presentes em apenas algumas linhagens, podendo conferir alguma vantagem adaptativa. Em Pseudomonas aeruginosa, até o momento foram caracterizadas pelo menos dezesseis ilhas genômicas e cada uma delas confere características diferentes a seus hospedeiros. Em P. aeruginosa UCBPP-PA14 (ou simplesmente PA14), encontram-se duas ilhas de patogenicidade denominadas PAPI-1 e PAPI-2, sendo a primeira a maior e a mais estudada, contendo 115 ORFs (“Open Reading Frame”, ou quadros abertos de leitura). Dentre estes, o gene int codifica uma integrase essencial para a excisão e integração de PAPI-1, e o gene soj é necessário para a manutenção da ilha na célula e é expresso apenas quando esta se encontra na forma epissomal. PAPI-1 codifica um provável sistema de secreção tipo IV (T4SS), similar ao do elemento móvel ICEHin1056, responsável pela transferência deste para outras bactérias. O objetivo deste trabalho foi identificar fatores genéticos e ambientais que contribuem para a transferência de PAPI-1 entre linhagens de P. aeruginosa. Foi observado que os mutantes por transposon nos genes PAPI-1 PA14_59860, PA14_59880, PA14_59920 e PA14_59940 têm a frequência de transferência de PAPI-1 diminuída, mas os genes interrompidos nesses mutantes não são essenciais para a excisão da ilha. Também foi mostrado que os reguladores percepção de quorum RhlR e MvfR têm influência na expressão do gene int, mas não de soj. O terceiro regulador de percepção de quorum, LasR, assim como a proteína H-NS MvaT, não tem influência na expressão de int e de soj. Ensaios de RT-PCR quantitativos mostraram que o choque térmico aumentou os níveis do mRNA de soj, mas não de int, corroborando dados previamente sugeridos pela literatura, que mostram uma maior freqüência de transferência de PAPI-1 nessas condições. Também foi analisado se o segundo mensageiro celular em bactérias, c-di-GMP, poderia contribuir para a excisão/manutenção de PAPI-1. Alterações nas concentrações deste segundo mensageiro pela superexpressão de proteínas responsáveis por sua síntese ou degradação não foram capazes de afetar a excisão/manutenção de PAPI-1. Houve diminuição na frequência de transferência de PAPI-1 a partir de linhagens doadoras superexpressando uma diguanilato ciclase ou uma fosfodiesterase de c-di-GMP, mas provavelmente este efeito não se deve aos níveis alterados desse segundo mensageiro. Em Xanthomonas axonopodis pv. citri 306 (XAC), uma região de 86 kb possui uma grande semelhança com PAPI-1 na organização dos genes. Além disso, possui uma série de ORFs relacionados aos genes “core” que definem uma família de ilhas genômicas sintênicas das quais PAPI-1 faz parte. Entretanto, os genes acessórios encontrados entre os blocos de genes conservados varia muito entre PAPI-1 e a região de XAC. Foi determinado que esta região de XAC não pode se excisar do cromossomo nas condições analisadas. Por fim, com o intuito de verificar as possíveis interações entre os produtos dos genes conservados em PAPI-1 e XAC, ensaios de duplo-híbrido foram realizados, porém não foi possível determiná-las, visto que apenas resultados falsos positivos foram obtidos. Este trabalho mostrou pela primeira vez que a percepção de quorum está envolvida com a expressão de soj e determinou uma extensa similaridade entre essa ilha e uma região do genoma de XAC / Bacterial genomes are extremely dynamic mostly because of horizontal gene transfer, a natural and fundamental process for evolution, adaptation and diversification of microorganisms. Genomic islands are large DNA segments acquired by horizontal gene transfer which are present only in a few strains and may confer some adaptative advantage. At least sixteen genomic islands have been characterized in Pseudomonas aeruginosa to date and each confers different characteristics to its host strain. P. aeruginosa UCBPP-PA14 (PA14) harbors two pathogenicity islands named PAPI-1 and PAPI-2. PAPI-1 is the largest one, carrying 115 open reading frames (ORFs). Among these, int codes for an integrase essential for PAPI-1 excision and integration, and soj is required for maintaining PAPI-1 in the cells, being expressed only when this island is in an episomal, circular form. PAPI-1 also harbors genes coding for a type four secretion system (T4SS) similar to the mobile element ICEHin1056, which is responsible for transferring this element to other bacteria. In this work, we show that transposon insertion in PAPI-1 genes PA14_59860, PA14_59880, PA14_59920 and PA14_59940 lowered the frequency of conjugation of PAPI-1 from PA14 to other bacteria, but those genes were not essential for PAPI-1 excision. Quorum sensing regulators RhlR and MvfR had a role in int expression, but did not alter soj transcription. The third quorum sensing regulator LasR, as well as the H-NS protein MvaT, did not alter both int and soj expression. Quantitative RT-PCR assays showed that cells incubated at heat shock conditions present higher levels of soj, mRNA, confirming published data that showed an increase in PAPI-1 transfer in these conditions. It was also analyzed whether the second messenger c-di-GMP would contribute to PAPI-1 excision/maintenance. Changes in the levels of this second messenger in cells overexpressing proteins responsible for its synthesis or degradation did not affect PAPI-1 excision and maintenance. A decrease in PAPI-1 transfer frequency was detected when those cells were used as donors in conjugation, but this effect cannot be attributed to the altered c-di-GMP levels. In Xanthomonas axonopodis pv. citri 306 (XAC), an 86 kb genome region shares similarity with PAPI-1 regarding gene homology and organization. It also carries ORFs related to the core genes that define a syntenic family of genomic islands that includes PAPI-1. Nevertheless, the accessory genes dispersed among the clusters of conserved genes are not related, when comparing PAPI-1 and this region in XAC. An epissomal form of this putative XAC island could not be detected in the conditions tested in this work. Finally, in order to verify interactions involving the conserved proteins in PAPI-1 and XAC, two hybrid assays were carried out, but only false positives results were obtained c-di-GMP c-di-GMP Genomic Island Horizontal Gene Transfer Ilhas Genômicas Percepção de Quorum Pseudomonas aeruginosa Pseudomonas aeruginosa Quorum Sensing Transferência Horizontal Xanthomonas axonopodis pv. citri 306 Xanthomonas axonopodis pv. citri 306
244	Collective regulation of the amoeboid motility : the role of short and long-range interactions in vegetative Dictyostelium discoideum / Régulation collective de la motilité amibienne : le rôle des interactions à courte et longue portée chez Dictyostelium discoideum à l'état végétatif D'Alessandro, Joseph 16 March 2016 (has links) La motilité cellulaire est fondamentale dans de nombreux processus physiologiques, qu’ils soient normaux ou pathologiques. Cependant, bien que ces derniers impliquent la plupart du temps de nombreuses cellules se mouvant en même temps, les effets des interactions entre cellules sur leur dynamique, à la fois individuelle et collective, restent assez mal connu. Dans cette thèse, j’ai utilisé Dictyostelium discoideum à l’état végétatif pour étudier cette régulation collective de la motilité. Je me suis principalement appuyé sur une analyse minutieuse de nombreuses trajectoires cellulaires dans des situations variées pour (i) caractériser un facteur sécrété qui régule négativement la motilité cellulaire (nature chimique, voie de signalisation, dynamique de sécrétion et de réponse) et (ii) analyser et modéliser quantitativement la dynamique d’étalement de colonie cellulaires de forme, dimension et densité contrôlées. Je décris enfin un phénomène d’agrégation dynamique observé lorsque les cellules sont placées à haute densité dans un milieu nutritif / Cell motility is fundamental in many physiological, either normal or pathological, phenomena. Yet, although these most often involve several cells moving at the same time, how the interactions between cells affect both individual and collective dynamics remains a poorly understood question. In this thesis, I used vegetative Dictyostelium discoideum cells as a model to study this collective regulation of the motility. I relied mainly on the thorough analysis of numerous cell trajectories in various situations to (i) characterise a secreted factor used to down-regulate the cells’ motility (biochemical nature, response pathway, secretion and response dynamics) and (ii) quantitatively analyse and model the dynamics of spreading cell colonies of controlled initial shape, size and density. Last, I describe a dynamic aggregation phenomenon that occurs when the cells are seeded at high density in a nutrient-rich medium Biophysique Physique statistique Matière active Motilité cellulaire Effets collectifs Détection du quorum Interactions cellule-cellule Biophysics Statistical physics Active matter Cell motility Collective effects Quorum sensing Cell-cell interactions 530.13
245	Fatores envolvidos com a mobilização de PAPI-1 / Factors involved with PAPI-1 mobilization Eliezer Stefanello 07 May 2010 (has links) Genomas bacterianos são extremamente dinâmicos e boa parte dessa dinâmica ocorre devido a transferência horizontal e aquisição de DNA exógeno, um processo natural e fundamental para a evolução, adaptação e diversificação dos microrganismos. Ilhas genômicas são grandes regiões do cromossomo bacteriano adquiridas por transferência horizontal e estão presentes em apenas algumas linhagens, podendo conferir alguma vantagem adaptativa. Em Pseudomonas aeruginosa, até o momento foram caracterizadas pelo menos dezesseis ilhas genômicas e cada uma delas confere características diferentes a seus hospedeiros. Em P. aeruginosa UCBPP-PA14 (ou simplesmente PA14), encontram-se duas ilhas de patogenicidade denominadas PAPI-1 e PAPI-2, sendo a primeira a maior e a mais estudada, contendo 115 ORFs (“Open Reading Frame”, ou quadros abertos de leitura). Dentre estes, o gene int codifica uma integrase essencial para a excisão e integração de PAPI-1, e o gene soj é necessário para a manutenção da ilha na célula e é expresso apenas quando esta se encontra na forma epissomal. PAPI-1 codifica um provável sistema de secreção tipo IV (T4SS), similar ao do elemento móvel ICEHin1056, responsável pela transferência deste para outras bactérias. O objetivo deste trabalho foi identificar fatores genéticos e ambientais que contribuem para a transferência de PAPI-1 entre linhagens de P. aeruginosa. Foi observado que os mutantes por transposon nos genes PAPI-1 PA14_59860, PA14_59880, PA14_59920 e PA14_59940 têm a frequência de transferência de PAPI-1 diminuída, mas os genes interrompidos nesses mutantes não são essenciais para a excisão da ilha. Também foi mostrado que os reguladores percepção de quorum RhlR e MvfR têm influência na expressão do gene int, mas não de soj. O terceiro regulador de percepção de quorum, LasR, assim como a proteína H-NS MvaT, não tem influência na expressão de int e de soj. Ensaios de RT-PCR quantitativos mostraram que o choque térmico aumentou os níveis do mRNA de soj, mas não de int, corroborando dados previamente sugeridos pela literatura, que mostram uma maior freqüência de transferência de PAPI-1 nessas condições. Também foi analisado se o segundo mensageiro celular em bactérias, c-di-GMP, poderia contribuir para a excisão/manutenção de PAPI-1. Alterações nas concentrações deste segundo mensageiro pela superexpressão de proteínas responsáveis por sua síntese ou degradação não foram capazes de afetar a excisão/manutenção de PAPI-1. Houve diminuição na frequência de transferência de PAPI-1 a partir de linhagens doadoras superexpressando uma diguanilato ciclase ou uma fosfodiesterase de c-di-GMP, mas provavelmente este efeito não se deve aos níveis alterados desse segundo mensageiro. Em Xanthomonas axonopodis pv. citri 306 (XAC), uma região de 86 kb possui uma grande semelhança com PAPI-1 na organização dos genes. Além disso, possui uma série de ORFs relacionados aos genes “core” que definem uma família de ilhas genômicas sintênicas das quais PAPI-1 faz parte. Entretanto, os genes acessórios encontrados entre os blocos de genes conservados varia muito entre PAPI-1 e a região de XAC. Foi determinado que esta região de XAC não pode se excisar do cromossomo nas condições analisadas. Por fim, com o intuito de verificar as possíveis interações entre os produtos dos genes conservados em PAPI-1 e XAC, ensaios de duplo-híbrido foram realizados, porém não foi possível determiná-las, visto que apenas resultados falsos positivos foram obtidos. Este trabalho mostrou pela primeira vez que a percepção de quorum está envolvida com a expressão de soj e determinou uma extensa similaridade entre essa ilha e uma região do genoma de XAC / Bacterial genomes are extremely dynamic mostly because of horizontal gene transfer, a natural and fundamental process for evolution, adaptation and diversification of microorganisms. Genomic islands are large DNA segments acquired by horizontal gene transfer which are present only in a few strains and may confer some adaptative advantage. At least sixteen genomic islands have been characterized in Pseudomonas aeruginosa to date and each confers different characteristics to its host strain. P. aeruginosa UCBPP-PA14 (PA14) harbors two pathogenicity islands named PAPI-1 and PAPI-2. PAPI-1 is the largest one, carrying 115 open reading frames (ORFs). Among these, int codes for an integrase essential for PAPI-1 excision and integration, and soj is required for maintaining PAPI-1 in the cells, being expressed only when this island is in an episomal, circular form. PAPI-1 also harbors genes coding for a type four secretion system (T4SS) similar to the mobile element ICEHin1056, which is responsible for transferring this element to other bacteria. In this work, we show that transposon insertion in PAPI-1 genes PA14_59860, PA14_59880, PA14_59920 and PA14_59940 lowered the frequency of conjugation of PAPI-1 from PA14 to other bacteria, but those genes were not essential for PAPI-1 excision. Quorum sensing regulators RhlR and MvfR had a role in int expression, but did not alter soj transcription. The third quorum sensing regulator LasR, as well as the H-NS protein MvaT, did not alter both int and soj expression. Quantitative RT-PCR assays showed that cells incubated at heat shock conditions present higher levels of soj, mRNA, confirming published data that showed an increase in PAPI-1 transfer in these conditions. It was also analyzed whether the second messenger c-di-GMP would contribute to PAPI-1 excision/maintenance. Changes in the levels of this second messenger in cells overexpressing proteins responsible for its synthesis or degradation did not affect PAPI-1 excision and maintenance. A decrease in PAPI-1 transfer frequency was detected when those cells were used as donors in conjugation, but this effect cannot be attributed to the altered c-di-GMP levels. In Xanthomonas axonopodis pv. citri 306 (XAC), an 86 kb genome region shares similarity with PAPI-1 regarding gene homology and organization. It also carries ORFs related to the core genes that define a syntenic family of genomic islands that includes PAPI-1. Nevertheless, the accessory genes dispersed among the clusters of conserved genes are not related, when comparing PAPI-1 and this region in XAC. An epissomal form of this putative XAC island could not be detected in the conditions tested in this work. Finally, in order to verify interactions involving the conserved proteins in PAPI-1 and XAC, two hybrid assays were carried out, but only false positives results were obtained c-di-GMP Ilhas Genômicas Percepção de Quorum Pseudomonas aeruginosa Transferência Horizontal Xanthomonas axonopodis pv. citri 306 c-di-GMP Genomic Island Horizontal Gene Transfer Pseudomonas aeruginosa Quorum Sensing Xanthomonas axonopodis pv. citri 306
246	Les régulateurs transcriptionnels Rgg. Confirmation de leur implication dans des phénomènes de quorum-sensing et identification de leurs cibles. Fleuchot, Betty 06 December 2011 (has links) (PDF) La découverte d'un contexte génétique chez les streptocoques - codant un petit peptide hydrophobe (SHP) et un régulateur transcriptionnel appartenant à la famille Rgg -, suivi de l'étude d'un de ces loci chez S. thermophilus LMD-9, a conduit à l'hypothèse que les protéines régulatrices Rgg en association avec une phéromone putative SHP pourraient intervenir dans un mécanisme de type quorum-sensing (QS) chez les bactéries à Gram positif. La première partie de ma thèse a consisté à confirmer cette hypothèse sur le locus shp/rgg1358 de S. thermophilus LMD-9, espèce contenant le plus grand nombre de systèmes SHP/Rgg dans son génome. Pour ceci, les étapes impliquées dans un mécanisme de QS ont été étudiées : la sécrétion, la maturation et la détection à une concentration seuil de la phéromone, sa réimportation à l'intérieur de la cellule, son interaction avec un régulateur transcriptionnel et enfin l'interaction de la protéine régulatrice à l'ADN. Par l'utilisation d'approches génétiques et biochimiques, nous avons démontré l'existence d'un nouveau mécanisme de QS impliquant pour la première fois un régulateur transcriptionnel Rgg et une phéromone SHP, importée à l'intérieur de la cellule par le transporteur d'oligopeptides AmiCDEF. Le rôle de la protéase membranaire, Eep, a également été démontré dans la maturation de la phéromone, dont la forme mature a été déterminée par spectrométrie de masse et validée in vivo. Dans un second temps, nous avons exploré la fonctionnalité de ce nouveau mécanisme sur d'autres loci shp/rgg, dans le but d'étudier l'existence d'éventuels phénomènes de cross-talk entre les bactéries. L'étude de nouveaux loci, en système hétérologue chez S. thermophilus LMD-9, a permis d'étendre la fonctionnalité du mécanisme à deux systèmes SHP/Rgg de streptocoques pathogènes, à savoir S. agalactiae et S. mutans. En parallèle à ce travail de caractérisation, l'identification des régulons des systèmes SHP/Rgg a été entreprise. La construction d'un arbre phylogénétique des protéines Rgg-like a permis d'identifier 68 systèmes SHP/Rgg, que nous avons classés en trois groupes. L'analyse des régions promotrices des gènes shp a conduit à l'identification d'un site putatif de liaison des protéines Rgg à l'ADN spécifiques de chaque groupe SHP/Rgg. Une approche in silico a ensuite été menée afin de rechercher, dans les génomes séquencés de streptocoques, les gènes cibles putatifs. Alors que des cibles proximales ont été détectées pour les groupes II et III, des cibles distales ont été identifiées dans les groupes I et II. Actuellement, la validation de certaines cibles est en cours au laboratoire. A l'avenir, ce travail pourrait permettre le développement de petits peptides permettant d'optimiser l'utilisation de S. thermophilus en industries laitières et de réduire la virulence des streptocoques pathogènes. Streptocoques Quorum sensing Régulateurs RNPP Régulateurs transcriptionnels Rgg Petits peptides hydrophobes Oligopeptide permease transporteur
247	Quorum Sensing Signals Produced by Heterotrophic Bacteria in Black Band Disease (BBD) of Corals and Their Potential Role in BBD Pathogenesis Bhedi, Chinmayee D. 30 June 2017 (has links) Black band disease (BBD) of corals is a temperature dependent, highly virulent, polymicrobial disease affecting reef-building corals globally. The microbial consortium of BBD is primarily comprised of functional physiological groups that include photosynthetic cyanobacteria, sulfate reducers, sulfide oxidizers and a vast repertoire of heterotrophic bacteria. Quorum sensing (QS), the cell-density dependent communication phenomenon in bacteria, is known to induce expression of genes for a variety of virulence factors in diseases worldwide. Microbes capable of QS release signals such as acyl homoserine lactones (AHLs) and autoinducer-2 (AI-2), which coordinate microbial interaction. The focus of the present study was to investigate the presence and potential role of QS in BBD pathogenicity, utilizing culture dependent and independent methodologies. Isolates across coral health states including BBD, were screened for production of QS signals, and AHL and AI-2 production capabilities were analyzed via LC-MS/MS. The effect of temperature on AHLs was also examined. Additionally, antimicrobial production capabilities of isolates were tested. BBD metagenomes were utilized to screen for sequences related to QS, antimicrobial synthesis, and antimicrobial resistance genes. BBD isolates represented a significantly higher proportion of isolates capable of producing QS signals in comparison to healthy coral isolates. Several AHLs produced by coral derived bacterial cultures were identified, and three AHLs, specifically 3OHC4, 3OHC5 and 3OHC6, showed a significant increase in production at an elevated temperature of 30 °C, which correlates with increased BBD incidence on reefs with increasing water temperature. Most of the BBD cultured isolates were identified as vibrios. Several sequences related to QS, antimicrobial synthesis and resistance genes were detected in the BBD metagenomes. Based on the findings of this study, a model for potential microbial interactions amongst BBD heterotrophs, centered around QS, is proposed. Taken together, the findings from this study provide a clearer understanding of the potential role of QS in BBD, and serve as the basis for further studies aimed at elucidating the pathogenesis of an intricate coral disease. black band disease corals quorum sensing acyl homoserine lactones metagenomics temperature coral disease secondary metabolites autoinducer-2 antimicrobial production Bacteriology Biology Biotechnology Marine Biology Microbial Physiology Microbiology Pathogenic Microbiology
248	Mathematical Models in Cell Cycle Biology and Pulmonary Immunity Buckalew, Richard L. 09 June 2014 (has links) No description available. Applied Mathematics Cellular Biology Immunology mathematical biology cell cycle pulmonary innate immunity immunity ODE model PDE model couples oscillators VAP ventilator associated pneumonia autonomous oscillation S cerevisiae quorum sensing cell cycle clustering dynamical systems
249	Identification of transcriptional regulators functions in the human fungal pathogen Candida albicans using functional genomics Khayat, Aline 01 1900 (has links) Candida albicans, une levure pathogène de l’humain, cause des infections envahissantes chez les individus immunodéprimés. C. albicans peut changer sa morphologie entre les formes levures et filamenteuses, un déterminant de virulence considérable qui est influencé par plusieurs facteurs environnementaux comme le pH, le sérum, les nutriments, et le farnesol, une molécule de la détection du quorum. Le génome de C. albicans a été séquencé et à date, plusieurs gènes codant des régulateurs de transcription (RT) restent incaracterisés. Basé sur des criblages à grande-échelle, il a été possible d’attribuer des phénotypes à certains des RT incaractérisés, cependant, leurs cibles traduisant ces phénotypes restent inconnues. Le but de cette thèse était d’étudier les fonctions biologiques de RT sélectionnés et d’établir des réseaux transcriptionnels chez C. albicans. J’ai utilisé des approches génétiques et génomiques afin d’identifier et de caractériser le regulon de ces RT, ce qui a permis de déterminer leur fonctions biologiques. Notre groupe avait identifié Fcr1p, un RT dont la délétion augmente la filamentation et la tolérance à plusieurs antifongiques. Cependant, le mécanisme sous-jacent reste inconnu. Dans le Chapitre 2, j’ai identifié le régulon d’Fcr1p et j’ai trouvé qu’il régule ses cibles de façon complexe étant en même temps un activateur et un répresseur d’expression de gènes. J’ai démontré que Fcr1p agit comme répresseur direct des gènes de l’assimilation et du métabolisme de l’azote. L’expression de plusieurs de ces cibles était dépendante d’Fcr1p en conditions d’épuisement d’azote. J’ai montrés que Fcr1p agit aussi comme répresseur indirect de gènes hyphe-spécifiques ainsi qu’un activateur indirect de transport et de métabolisme du carbone et de gènes levure-spécifiques. De plus, la suréxpression d’Fcr1p abolit la filamentation sur le milieu Spider, confirmant que c’est un répresseur de filamentation. Dans le Chapitre 3, j’ai décris un crible génétique basé sur un principe de co-culture pour identifier des mutants de RT défectueux en production de farnesol. Conséquemment, les RT Ada2p, Cas5p, Fgr15p, Cas1p, et Rlm1p, impliqués dans le maintien de la paroi cellulaire, ont été identifiés. La quantification du farnesol intracellulaire de ces mutants a confirmé que le défaut observé peut être attribué à un défaut de la biosynthèse de farnesol plutôt qu’à un défaut de sécrétion de celui-ci. Pour comprendre le mécanisme responsable de ce défaut, nous avons commencé par caractériser le régulon de Cas5p par des analyses de profilages d’expression et de localisation. J’ai montré que Cas5p se lie à des gènes impliqués dans le catabolisme des hydrocarbures et la production d’énergie. Cas5p induit aussi des gènes impliqués dans le catabolisme des hydrocarbures et des lipides et réprime des gènes impliqués dans le métabolisme primaire, montrant que Cas5p régule plusieurs voies métaboliques, notamment celle du carbone. En plus des fonctions d’Ada2p et Rlm1p dans la liaison et/ou la régulation de gènes du catabolisme des hydrocarbures, nos résultats appuient avec la proposition que le farnesol constitue une traduction du métabolisme du carbone cellulaire. Dans l’ensemble, ces résultats ont aidé à élucider le rôle d’Fcr1p ainsi que 5 autres RT dans la régulation de voies métaboliques fondamentales influençant le dimorphisme, un attribut crucial de la virulence chez C. albicans. / Candida albicans, an important human fungal pathogen, causes life-threatening invasive infections in immuno-compromised individuals. It switches between yeast and filamentous forms. This dimorphism is a considerable virulence attribute and one that is influenced by many environmental factors, such as pH, serum, nutrients and farnesol, a quorum sensing molecule. The genome of C. albicans has been sequenced and to date, many of the genes encoding transcriptional regulators (TRs) remain uncharacterized. Based on large-scale screens, it was possible to assign phenotypes to some of the uncharacterized TRs, however the targets of these TRs that mediate these phenotypes remain to be identified. The aim of this thesis work was to understand the normal biological function of selected TRs and construct transcriptional networks in C. albicans. I used genetic and genomic approaches to identify and characterize the regulon of these TRs, which helped to define their biological functions. Our group has previously identified Fcr1p, a zinc cluster TR whose deletion increases cell tolerance to multiple drugs and enhances filamentation. However, the mechanism by which it mediates these phenotypes is still unknown. In Chapter 2, I identified the regulon of Fcr1p and found that it regulates its targets in a complex manner since it can act both as an activator and as a repressor of gene expression. I have shown that Fcr1p acts as a direct negative regulator of genes involved in nitrogen source assimilation and metabolism. The Fcr1p-dependent expression of a number of its targets also occurs under nitrogen starvation conditions. Results also showed that Fcr1p is an indirect negative regulator of hyphal-specific genes, and an indirect positive regulator of carbon source transport and metabolism, as well as yeast-specific genes. Furthermore, Fcr1p overexpression abrogates filamentation on Spider medium confirming that it is a negative regulator of filamentation. In Chapter 3, I describe a genetic screen based on a co-culture assay with A. nidulans to identify TR mutants defective in farnesol production. Our results identified Ada2p, Cas5p, Fgr15p, Cas1p, and Rlm1p, five TRs involved in cell wall integrity. Intracellular farnesol quantification in these mutants confirmed that the observed defect in farnesol production could be attributed to impairment in farnesol biosynthesis rather than export of this molecule. To get an insight into the molecular mechanism responsible for this defect, we started by identifying the regulon of Cas5p using expression and location profiling. Results showed that Cas5p binds genes involved in carbohydrate catabolism and energy production. Cas5p also upregulates genes involved in carbohydrate and lipid catabolism and downregulates genes involved in primary metabolism, indicating that Cas5p is involved in the regulation of many pathways, with a clear involvement in carbon metabolism. Coupled to the known function of Ada2p and Rlm1p in binding and/or regulating genes involved in carbohydrate catabolism, our results support the proposition that farnesol is a metabolic read-out of the cell carbon metabolic activity. Taken together, these results helped elucidate the role of Fcr1p as well as five other TRs in the regulation of central metabolic pathways that influence morphological switching, a crucial attribute of C.albicans virulence. Candida albicans azote carbone métabolisme assimilation farnesol détection du quorum filamentation régulation transcriptionnelle génomique fonctionnelle nitrogen carbon metabolism quorum sensing transcriptional regulation functional genomics
250	Gene expression control for synthetic patterning of bacterial populations and plants Boehm, Christian Reiner January 2017 (has links) The development of shape in multicellular organisms has intrigued human minds for millenia. Empowered by modern genetic techniques, molecular biologists are now striving to not only dissect developmental processes, but to exploit their modularity for the design of custom living systems used in bioproduction, remediation, and regenerative medicine. Currently, our capacity to harness this potential is fundamentally limited by a lack of spatiotemporal control over gene expression in multicellular systems. While several synthetic genetic circuits for control of multicellular patterning have been reported, hierarchical induction of gene expression domains has received little attention from synthetic biologists, despite its fundamental role in biological self-organization. In this thesis, I introduce the first synthetic genetic system implementing population-based AND logic for programmed hierarchical patterning of bacterial populations of Escherichia coli, and address fundamental prerequisites for implementation of an analogous genetic circuit into the emergent multicellular plant model Marchantia polymorpha. In both model systems, I explore the use of bacteriophage T7 RNA polymerase as a gene expression engine to control synthetic patterning across populations of cells. In E. coli, I developed a ratiometric assay of bacteriophage T7 RNA polymerase activity, which I used to systematically characterize different intact and split enzyme variants. I utilized the best-performing variant to build a three-color patterning system responsive to two different homoserine lactones. I validated the AND gate-like behavior of this system both in cell suspension and in surface culture. Then, I used the synthetic circuit in a membrane-based spatial assay to demonstrate programmed hierarchical patterning of gene expression across bacterial populations. To prepare the adaption of bacteriophage T7 RNA polymerase-driven synthetic patterning from the prokaryote E. coli to the eukaryote M. polymorpha, I developed a toolbox of genetic elements for spatial gene expression control in the liverwort: I analyzed codon usage across the transcriptome of M. polymorpha, and used insights gained to design codon-optimized fluorescent reporters successfully expressed from its nuclear and chloroplast genomes. For targeting of bacteriophage T7 RNA polymerase to these cellular compartments, I functionally validated nuclear localization signals and chloroplast transit peptides. For spatiotemporal control of bacteriophage T7 RNA polymerase in M. polymorpha, I characterized spatially restricted and inducible promoters. For facilitated posttranscriptional processing of target transcripts, I functionally validated viral enhancer sequences in M. polymorpha. Taking advantage of this genetic toolbox, I introduced inducible nuclear-targeted bacteriophage T7 RNA polymerase into M. polymorpha. I showed implementation of the bacteriophage T7 RNA polymerase/PT7 expression system accompanied by hypermethylation of its target nuclear transgene. My observations suggest operation of efficient epigenetic gene silencing in M. polymorpha, and guide future efforts in chassis engineering of this multicellular plant model. Furthermore, my results encourage utilization of spatiotemporally controlled bacteriophage T7 RNA polymerase as a targeted silencing system for functional genomic studies and morphogenetic engineering in the liverwort. Taken together, the work presented enhances our capacity for spatiotemporal gene expression control in bacterial populations and plants, facilitating future efforts in synthetic morphogenesis for applications in synthetic biology and metabolic engineering. 572.8

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